Background

Candida glabrata is a pathogenic yeast of increasing medical concern. It has been regarded as asexual since it was first described in 1917, yet phylogenetic analyses have revealed that it is more closely related to sexual yeasts than other Candida species. We show here that the C. glabrata genome contains many genes apparently involved in sexual reproduction.

Results

By genome survey sequencing, we find that genes involved in mating and meiosis are as numerous in C. glabrata as in the sexual species Kluyveromyces delphensis, which is its closest known relative. C. glabrata has a putative mating-type (MAT) locus and a pheromone gene (MFALPHA2), as well as orthologs of at least 31 other Saccharomyces cerevisiae genes that have no known roles apart from mating or meiosis, including FUS3, IME1 and SMK1.

Conclusions

We infer that C. glabrata is likely to have an undiscovered sexual stage in its life cycle, similar to that recently proposed for C. albicans. The two Candida species represent two distantly related yeast lineages that have independently become both pathogenic and 'asexual'. Parallel evolution in the two lineages as they adopted mammalian hosts resulted in separate but analogous switches from overtly sexual to cryptically sexual life cycles, possibly in response to defense by the host immune system.

The genus Candida consists of ascomycete yeast species that lack an apparent sexual (teleomorph) stage in their life cycle and seem to reproduce only mitotically. However, data from the C. albicans genome project has recently led researchers to question the asexuality of that species. C. albicans was found to have a mating type-like (MTL) locus similar to the Saccharomyces cerevisiae MAT locus [1]. Natural isolates of C. albicans are diploid MTLa/MTLα heterozygotes, similar to diploid S. cerevisiae but unable to sporulate. By genetic engineering to create MTLa and MTLα hemizygotes, C. albicans was induced to mate in the laboratory and in infected mice, forming tetraploids [2,3]. In addition, Miller and Johnson [4] showed that C. albicansMTL hemizygotes undergo phenotypic switching between the common 'white' form and an 'opaque' form that is a million-fold more active in mating. Further analysis of the almost-complete genome sequence of C. albicans revealed that it contains homologs of most of the S. cerevisiae genes involved in the key sexual processes of meiosis and sporulation as well as mating [5]. These findings have led to the hypothesis that the life cycle of C. albicans includes a cryptic sexual phase, which perhaps is utilized only occasionally or under particular environmental conditions [6] - infrequently enough not to have been detected during more than a century of research into C. albicans, but frequently enough to cause evolutionary conservation of the genes involved in the sexual process. Interestingly, sexual forms of some other Candida species were identified long ago by mycologists but their significance has often gone unrecognized by molecular biologists because the anamorphs and teleomorphs are assigned different names - for example, the sexual form of Candida krusei is called Issatchenkia orientalis [7,8].

Medically, C. albicans is still the major fungal agent of human disease, but C. glabrata is a species of growing concern. The incidence of C. glabrata infections, particularly in the bloodstream, has risen alarmingly over the past decade [9,10]. It has also gained much attention since the discovery of its inherently low susceptibility to the drug fluconazole [11]. The genome of C. glabrata appears to be haploid whereas C. albicans is diploid [12,13]. But similarly to C. albicans, C. glabrata also undergoes phenotypic switching [14,15], raising the interesting question of whether it too may have an undiscovered teleomorph form.

In phylogenetic trees drawn from rDNA sequences, most Candida species including C. albicans fall into one monophyletic group, whereas C. glabrata is much more closely related to S. cerevisiae than to the C. albicans group (Figure 1 and [16,17,18]). Therefore, the 'asexual' life cycles of C. glabrata and C. albicans arose independently from sexual ancestors [16,19]. Phylogenetic analysis also showed unexpectedly that C. glabrata's closest relative is Kluyveromyces delphensis, a sexual species [17,18]. C. glabrata is a commensal resident of the human intestinal tract and an opportunistic pathogen [20,21], whereas K. delphensis was first isolated from dried figs [22] and is often found associated with Drosophila willistoni [23]. The type strain of K. delphensis is homothallic and therefore probably diploid. It has been studied very little at the molecular level.

The aim of the present study was to use genome survey sequencing (GSS) to characterize the genomic differences between the closely related asexual C. glabrata and the sexual K. delphensis. However, we find that there are no significant differences between the gene repertoires of these species. C. glabrata has many genes involved in mating, meiosis and sporulation, including a pheromone gene and a putative mating-type locus. This leads us to propose that, like C. albicans, it must have an undiscovered sexual phase in its life cycle.

Genome survey sequencing of C. glabrata and K. delphensis

We constructed plasmid libraries with random genomic inserts of 7-15 kilobases (kb) from C. glabrata and K. delphensis and sequenced both ends of about 3,000 plasmids (> 3 megabases (Mb) of primary sequence data, or approximately 0.2× genome coverage) from each species. Phylogenetic analysis of the combined complete 5S, 18S, 5.8S and 26S rDNA sequences from yeasts (Figure 1) confirms that C. glabrata and K. delphensis are each other's closest known relatives [17,18]. The phylogenetic tree also confirms that C. glabrata is more closely related to S. cerevisiae than to C. albicans, indicating that the two Candida species originated independently from sexual ancestors.

Assembled sequence contigs from C. glabrata and K. delphensis were searched against the complete set of S. cerevisiae proteins using FASTY reciprocal best hits to identify putative orthologs (see Materials and methods). The results of the genome surveys of the two species should be roughly comparable to one another, because the same methods and similar numbers of clones were used in both cases. The genomes can be assumed to be similar in size [24,25], and the two species are equally distantly related to S. cerevisiae. Indeed, they yielded similar numbers of sequence contigs (4,481 from C. glabrata, 4,202 from K. delphensis) and similar numbers of putative genes with unambiguous S. cerevisiae orthologs (1,941 and 2,057, respectively).

Gene functions in C. glabrata and K. delphensis were inferred from the known functions of their S. cerevisiae orthologs, using the 'cellular role' categories of the Yeast Proteome Database (Table 1). Orthologs were found for approximately 40% of the S. cerevisiae genes involved in most cellular roles, reflecting the level of GSS coverage. The numbers of genes found in C. glabrata and K. delphensis for each cellular role are highly similar (Table 1), and the two genomes are not significantly different in any of the 42 categories (p > 0.05 by χ2 test). Importantly, C. glabrata does not have significantly fewer genes than K. delphensis in the categories of mating response and meiosis, which relate to sexual functions.

Table 1

Numbers of C. glabrata and K. delphensis orthologs found in different YPD 'cellular role' categories

YPD 'cellular role' categories

C. glabrata

K. delphensis

CG/SC*

KD/SC†

S. cerevisiae‡

Aging

16

15

0.41

0.38

39

Amino acid metabolism

92

96

0.42

0.44

217

Carbohydrate metabolism

70

84

0.28

0.33

254

Cell adhesion

1

3

0.25

0.75

4

Cell cycle control

96

91

0.45

0.43

213

Cell polarity

91

97

0.42

0.45

216

Cell stress

98

114

0.30

0.34

331

Cell structure

51

51

0.43

0.43

120

Cell wall maintenance

68

75

0.37

0.41

184

Chromatin/chromosome structure

111

119

0.41

0.43

274

Cytokinesis

21

26

0.53

0.65

40

Differentiation

36

25

0.35

0.24

104

DNA repair

59

76

0.38

0.49

154

DNA synthesis

53

55

0.51

0.53

104

Energy generation

107

103

0.37

0.36

290

Lipid and sterol metabolism

76

99

0.37

0.48

206

Mating response§

45

54

0.34

0.41

132

Meiosis§

56

56

0.38

0.38

147

Membrane fusion

15

16

0.38

0.40

40

Mitochondrial transcription

3

4

0.60

0.80

5

Mitosis

72

73

0.49

0.50

147

Nuclear-cytoplasmic transport

49

48

0.53

0.52

92

Nucleotide metabolism

26

35

0.27

0.37

95

Other

27

26

0.47

0.46

57

Other metabolism

62

71

0.32

0.37

192

Phosphate metabolism

8

9

0.31

0.35

26

Pol I transcription

14

14

0.47

0.47

30

Pol II transcription

148

158

0.39

0.41

384

Pol III transcription

15

19

0.38

0.49

39

Protein complex assembly

22

20

0.47

0.43

47

Protein degradation

86

90

0.47

0.49

183

Protein folding

33

42

0.36

0.46

91

Protein modification

99

106

0.40

0.43

246

Protein synthesis

99

106

0.27

0.28

373

Protein translocation

37

31

0.43

0.36

87

Recombination

29

39

0.33

0.44

88

RNA processing/modification

126

144

0.45

0.51

280

RNA splicing

44

50

0.38

0.43

116

RNA turnover

19

28

0.37

0.54

52

Signal transduction

54

55

0.40

0.41

135

Small molecule transport

138

144

0.34

0.35

407

Vesicular transport

136

146

0.45

0.48

305

Average

0.40

0.44

*Proportion of S. cerevisiae genes in the category with orthologs in C. glabrata. †Proportion of S. cerevisiae genes in the category with orthologs in K. delphensis. ‡Number of S. cerevisiae genes assigned to the category in the YPD database. §Lists of the mating response and meiosis genes identified in C. glabrata and K. delphensis are given in the additional data file.

Mating pathway genes

We identified C. glabrata orthologs of many genes in the S. cerevisiae mating response pathway including the Ste11, Ste7 and Fus3 kinases and the Ste12 transcription factor (Figure 2). Because some components of the mating pathway also participate in other pathways (such as filamentous growth) that might legitimately be expected to be present in an asexual organism, we focus here on genes that have no other known functions apart from mating. The GSS data identified C. glabrata orthologs of 13 S. cerevisiae genes that may be involved exclusively in mating (Table 2). These include an α-factor pheromone gene (MFALPHA2 [26]), STE13, whose sole function appears to be maturation of prepro-α-factor [27], and STE6, whose only known role is in a-factor export [28]. The complete C. glabrata MFALPHA2 gene was sequenced and codes for a signal peptide and three repeats of a candidate mature pheromone sequence WHWV(R/K)(L/I)RKGQGLF (single-letter amino-acid notation) flanked by processing sites for Kex2 [29], Kex1 and Ste13 proteases. The ortholog in K. delphensis was also sequenced and has four copies of the sequence WHWLSVRPGQPIY. The two precursor proteins share 49% sequence identity.

Figure 2

Model of the S. cerevisiae pheromone response pathway (adapted from [30]). Genes whose orthologs were identified in C. glabrata are indicated in gray.

Table 2

Mating-specific S. cerevisiae genes with orthologs in C. glabrata

Gene

Function

MFALPHA2

Mating pheromone α-factor

STE13

Peptidase, α-factor processing

STE6

Exporter of a-factor

FIG4

Lipid phosphatase, pheromone induced

FAR1

Inhibitor of Cdc28-Cln1/2 kinase complexes

CDC24

GTP-GDP exchange factor for Cdc42

SGV1

Kinase, pheromone adaptation

AKR1

Negative regulator in the pheromone response pathway

FUS3

Kinase, activates Ste12 and Far1

KAR5

Required for nuclear membrane fusion during karyogamy

LSG1

Required for normal morphology, mating and sporulation

OPY2

Overproduction causes insensitivity to α-factor arrest

SAG1

α-Agglutinin

C. glabrata appears capable of responding to pheromones as well as synthesizing them, because it has genes for the polarity-establishment proteins Far1 and Cdc24 [30], for Sgv1 (a kinase acting in the pheromone adaptation pathway [31]), and Akr1 (a protein with an inhibitory effect on the pheromone signal transduction pathway [32]). At the end of the signal transduction cascade it has orthologs of Fus3 (the final MAP kinase in the mating response pathway, which activates Ste12 and Far1 [33]), as well as the nuclear fusion protein Kar5 [34].

We identified putative mating-type (MAT) loci in both C. glabrata and K. delphensis, containing orthologs of the S. cerevisiae genes for the α1 transcription activator and the α2 repressor (MATALPHA1 and MATALPHA2, respectively), oriented divergently (Figure 3). As expected from the species phylogeny, the level of amino-acid sequence identity between S. cerevisiae and C. glabrata (38% in α1, and 40% in α2) is greater than that between S. cerevisiae and K. lactis or C. albicans in the same proteins [1,35]. Between C. glabrata and K. delphensis, there is 59% amino-acid sequence identity in α1 and 76% in α2.

Figure 3

Gene organization (not to scale) around the MAT locus of S. cerevisiae and the putative MAT loci of K. delphensis and C. glabrata. Dashed horizontal lines indicate the extents of the clones sequenced.

In K. delphensis the α2 and α1 genes are flanked on one side by a series of five genes whose orthologs are beside the MAT locus on S. cerevisiae chromosome III (Figure 3), in the same arrangement except that K. delphensis lacks PHO87. These genes include BUD5, which is almost twice as large in K. delphensis as in S. cerevisiae (1,241 amino acids versus 642). The predicted KdBud5 protein includes an extra SH3 domain near its amino terminus, giving it an overall structure more similar to Cdc25 [36]. On the other side of the α2 and α1 genes in K. delphensis there is a series of five genes whose orthologs are on S. cerevisiae chromosome XII, beginning with YLR186W (EMG1 [37]). The same breakpoint between chromosome III and chromosome XII orthologs is also seen in C. glabrata (Figure 3). It therefore seems likely that a chromosomal rearrangement occurred on the right-hand side of the MAT locus either in an ancestor of K. delphensis and C. glabrata, or in an ancestor of S. cerevisiae. Interestingly, the coding regions of the α1 gene and EMG1 overlap by 28 nucleotides at their 3' ends in both K. delphensis and C. glabrata.

Meiotic genes

The GSS data from C. glabrata also identified orthologs of many S. cerevisiae genes involved in meiosis, a central step in the sexual cycle that leads ultimately to the production of gametes (sporulation). We found C. glabrata orthologs of 19 S. cerevisiae genes whose only known functions are in meiosis or sporulation (Table 3), including the master regulatory switch gene IME1 [38]. S. cerevisiaeIME1 expression is induced by the a1/α2 heterodimer representing the genetic signal from a diploid cell, in combination with nutritional signals. We found C. glabrata orthologs of MCK1 and RIM9, which are inducers of IME1 expression, and UME6 which negatively regulates meiosis-specific genes during vegetative growth but is converted into an activator of early meiosis genes when Ime1 is present [39,40]. C. glabrata also has orthologs of IME2, which can promote sporulation in the absence of IME1 [41], and IDS2 and RIM4, whose products promote Ime2-dependent activation of many downstream targets [42,43].

Table 3

Meiosis-specific S. cerevisiae genes with orthologs in C. glabrata

Gene

Function

IME1

Master regulatory switch of meiosis

MCK1

Kinase required for maximal IME1 expression

RIM9

Stimulates expression of IME1

IME2

Kinase, stimulates meiotic gene expression

UME6

Transcriptional regulator of meiotic genes

RIM4

Activation of sporulation-specific genes

IDS2

Ime2-dependent signaling protein

MUM2

Required for premeiotic DNA synthesis and sporulation

HOP2

Prevents nonhomologous synapsis in meiosis

MSH4

Meiosis-specific MutS homolog, recombination

SPO1

Required for spindle body duplication

SPO22

Required for meiotic chromosome segregation

CSM1

Required for meiotic chromosome segregation

CSM3

Required for meiotic chromosome segregation

SMK1

Sporulation-specific MAP kinase

DIT1

Dityrosine biosynthesis enzyme

SPO75

Required for spore and ascus formation

SMA2

Required for proper prospore membrane formation

SPS2*

Putative prospore membrane protein

*We are not certain whether plasmid CG4206 contains an ortholog of SPS2 or the similar gene YCL048W, but we have included it in the table because both SPS2 and YCL048W encode prospore membrane proteins induced during sporulation [70].

C. glabrata has orthologs of RIM4 and MUM2, both of which are needed for premeiotic DNA replication [44,45], and HOP2, which acts to prevent synapsis between nonhomologous chromosomes [46]. We also found MSH4, which is implicated in synaptonemal complex formation and meiotic recombination [47]. The presence of these genes suggests that critical events required for the unique process of reductional division during meiosis I, such as recombination and chromosome synapsis, occur in C. glabrata.

Similarly, we found orthologs of genes involved in the middle and late stages of meiosis. The middle-stage genes include SPO1, a phospholipase B homolog that promotes spindle-body duplication exclusively during meiosis [48], and SPO22, CSM1 and CSM3 which are less well characterized but show meiosis-specific expression with deletion mutants exhibiting varying degrees of chromosome missegregation [49]. C. glabrata also has a homolog of SMK1, which in S. cerevisiae encodes a MAP kinase involved in a sporulation-specific signal transduction cascade, necessary for proper spore morphogenesis and full expression of late meiotic genes [50,51]. Another surprising finding is an ortholog of DIT1, which is required for dityrosine biosynthesis [52]. In yeasts, the dimerized amino acid dityrosine has only been found on the outer surface layer of the ascospore wall but not in vegetative cell walls [53]. The maintenance of these genes in C. glabrata is highly indicative of an ability to sporulate.

The results from survey sequencing of the C. glabrata and K. delphensis genomes show that they have very similar repertoires of genes in all categories of cellular roles (Table 1), including mating and meiosis. More detailed analysis showed that C. glabrata has orthologs of at least 31 genes that in S. cerevisiae have no known functions apart from mating or meiosis (Tables 2 and 3), and that it has intact genes for α-factor and a putative mating-type locus. Together, these results suggest that C. glabrata has an undiscovered sexual cycle. Although it is possible that future studies in S. cerevisiae will discover new roles for some of these genes other than in mating or meiosis, it seems more reasonable to propose that C. glabrata has a sexual cycle than to propose that it is asexual and that all 31 genes have been preserved in its genome because they have undiscovered roles in nonsexual processes. The compact nature of yeast genomes makes it unlikely that all the sexual genes we identified by GSS are pseudogenes, and the MFALPHA2, MATALPHA1 and MATALPHA2 genes certainly are not pseudogenes.

Even though we did not find orthologs of some other genes that are central to mating (for example, STE2/STE3 and MFA1 [54]) or meiosis (for example, NDT80), it should be noted that the genome was only surveyed to 0.2× sequence coverage, so that only 1,941 genes (roughly one-third of the expected number of genes in the genome) were detected in this study. It is interesting that C. glabrata has orthologs of MFALPHA2 and IME1, which were not found in C. albicans [5]. However, this is possibly just due to extensive sequence divergence, rather than gene loss, in C. albicans. The complete sequence of C. glabrata Ime1 has only 27% amino-acid sequence identity to S. cerevisiae Ime1. Very recently, a candidate C. albicans pheromone gene was described [55,56].

Despite the evolutionary distance between them (Figure 1) and gross differences such as the fact that C. glabrata is haploid whereas C. albicans is diploid, there are remarkable parallels between the evolution of C. glabrata and C. albicans. The two species have evolved independently from sexually reproducing yeast ancestors that are unlikely to have been pathogenic, because the majority of lineages in this phylogenetic group are not pathogenic (Figure 1). Thus, in becoming human pathogens, both C. glabrata and C. albicans have adopted a lifestyle where the sexual phase is hidden. Miller and Johnson [4] proposed that, in C. albicans, this is because the white (asexual) form survives better in the mammalian host. By analogy, it is tempting to speculate that one of the forms produced by phenotypic switching in C. glabrata [14,15] might be mating-competent. It is interesting to note that in other species of Candida for which sexual forms (teleomorphs) have been identified, such as Candida krusei, the form isolated in clinical settings is invariably the asexual one [7,8]. We hypothesize that having a sexual cycle may be essential for the long-term evolutionary viability of all yeast species because of the evolutionary advantages conferred by recombination [57,58], but that mating confers a disadvantage on those individuals that mate because they are somehow more vulnerable to the host's immune response. The result of these opposing forces seems to have been the evolution of cryptically sexual pathogens in which the frequency of mating in the population has been reduced to a low but optimal level.

The type strains of C. glabrata (CBS 138) and K. delphensis (CBS 2170) were purchased from the Centraalbureau voor Schimmelcultures (Utrecht, Netherlands). High-molecular-weight DNA was prepared using standard procedures and partially digested with Sau3AI. Fragments in the size range 7-15 kb were isolated and used to make random genomic libraries in the low copy number Escherichia coli vector pMCL210 (AGOWA, Germany). Sequences were obtained from both ends of the insert for 2,939 C. glabrata (CG) and 2,974 K. delphensis (KD) clones, with a further 449 CG and 290 KD clones sequenced successfully from one end only. The average lengths of sequence reads used for analysis were 548 base-pairs (bp) (CG) and 515 bp (KD). Representation of mitochondrial DNA in the libraries appeared to be very low, even though we did not take any specific measures to exclude it. After data analysis, the inserts of selected plasmid clones were sequenced completely on both strands by primer walking. Sequences have been deposited in GenBank with accession numbers BZ293019-BZ299345 (C. glabrata GSS), BZ299346-BZ305583 (K. delphensis GSS), AY181247-AY181250 (complete sequences of MAT and MFALPHA2 loci), and AJ535506 (C. glabrata IME1).

Trace files from the random genomic clones were base-called using PHRED [59,60] and vector clipping was done by CROSS_MATCH. Clipped sequences shorter than 100 bp were discarded from the dataset. Contigs were assembled using PHRAP with the original trace quality files and are available on request. Contigs were filtered to eliminate mitochondrial DNA as well as known repetitive sequences such as rDNA and Ty elements, which may cause misassembly. This was achieved using the contigs as queries in BLASTN and BLASTX searches [61] against the relevant S. cerevisiae sequences. Any contig with a significant expect value (E-value) of < 1e-5 was excluded from ortholog assignment.

We used a recent annotation of the S. cerevisiae genome [62], containing 5,583 annotated proteins (excluding 'very hypothetical' proteins and pseudogenes), downloaded from [63]. Orthologs of these genes in the C. glabrata and K. delphensis filtered contigs were identified using FASTY version 3.4t05 [64], after a low complexity masking step using the NSEG and PSEG programs [65]. For any gene-sized region in a contig, we considered the S. cerevisiae protein with the strongest FASTY hit to be the ortholog, provided that the E-value for this hit was < 1e-5 and was more than 1e3 times lower than the E-value for the second-best hit to the same region of the contig. For each ortholog identified, its function in S. cerevisiae was examined using the 'cellular role' categories of the Yeast Proteome Database (YPD) of the Incyte BioKnowledge Library [66]. It should be noted that in this functional annotation scheme, a single protein can be classified into more than one cellular role. While we adhered strictly to the YPD classification of genes in our initial analyses (Table 1), we also discovered some genes that can be reclassified on the basis of the literature (for example, SPS2 was classified under 'differentiation' in YPD but was found to be meiosis-specific on further examination) and included these reclassified genes in Tables 2 and 3.

Among the full set of contigs, those that contained rDNA sequences were identified. These were used in conjunction with publicly available rDNA sequences, isolated from the C. glabrata and K. delphensis type strains, to create the complete rDNA repeating unit for both species. The two rDNA sequences were combined with those from 14 other hemiascomycete yeast species used in our previous study [67] and aligned using T_COFFEE [68]. Phylogenetic trees were constructed using the NJ method as implemented in CLUSTALW [69].

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